AU596810B2 - A bacterial methionine n-terminal peptidase - Google Patents

Description

FORM 10 .596810 SPRUSON FERGUSON COMMONWEALTH OF AUSTRALIA PATENTS ACT 1952 COMPLETE SPECIFICATION

(ORIGINAL)

FOR OFFICE USE: Class Int. Class Complete Specification Lodged: Accepted: Published: ItuIS Jihaon Ulnsm U11IM ametidments ade uxWar Smbctin 49.

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z Priority: DC 0 O 00 a 0000 0 0 0 00 0 00 0 a a 0 a 00 a 0 *0L0 a aa a 0 0000 o 00 a aa Related Art: Name of Applicant: Address of Applicant: Actual Inventor(s): Address for Service: CETUS CORPORATION 1400 Fifty-Third Street, Emeryville, California 94608, United States of America ARIE BEN-BASSAT, KEITH ALAN BAUER, SHING CHANG and SHENG-YUNG CHANG Spruson Ferguson, Patent Attorneys, Level 33 St Martins Tower, 31 Market Street, Sydney, New South Wales, 2000, Australia a Oat 0 a a aa a aoO9 a a a f 00 0 0 0 0 0 0 Complete Specification for the invention entitled: "A BACTERIAL METHIONINE N-TERMINAL PEPTIDASE" The following statement is a full description of this invention, including the best method of performing it known to us A BACTERIAL METHIONINE N-TERMINAL PEPTIDASE Abstract Methods of obtaining N-terminal methionine-free proteins are described. The methods employ a novel enzyme, E. coli methionine aminopeptidase either in vitro or in vivo. For in vivo application. plasmid-borne DNA encoding the peptidase is transformed into a bacterial host which produces the desired protein.

is Q0000 200 030 A BACTERIAL METHIONINE N-TERMINAL PEPTIDASE Technical Field The invention r;,lates to production of proteins, especially foreign proteins, lacking an N-terminal methionine. in bacterial systcms using recobinant techniques. More specifically, it relates to a peptidase specific for N-terminal methionine which can be used in vitro or used to create a superior bacterial host containing elevated levels of peptidase for complete processing of mature prote~ns in these systems.

Background Art Production of foreign proteins in bacterial hosts is now well established. In relatively standard procedures, the gene sequence encoding the desired protein is placed under the control of regulatory sequences indigenous to or compatible with the host and transformed into the host bacterium. In general, there are three major ways in which this can be accomplished: (1) 0 the DNA encoding the desired protein can be fused in reading frame with a bacterial gene already under the 2control of the bacterial regulatory sequences to obtain a "fusion protein"; the desired coding sequences can 0, he fused in reading frame with an operable leader sequence resulting in a secreted protein; or the desired coding sequence is placed immediately downstream from an ATG start codon which results in "direct" expression to obtain the "mature" protein. In this last instance, the mature protein is not secreted but is found in an intracellular location, often as a refractile or inclusion body.

It is often left unstated, but well recognized by practitioners in the art, that the mature protein formed by the direct expression of ATG-preceded coding sequences frequently bears an N-terminal methionine which is the translation product of the ATG. Depending on the particular recombinant protein, and on the circumstances of its production, more or less of- it may be processed in the cell to remove this N-terminal Met residue, but, in general, at least some, and usually a substantial portion of the recombinant protein produced does bear this unwanted foreign residue. Its presence is not completely harmless. When the resulting proteins are used therapeutically, what would ordinarily be an autologous protein to the recipient (for example, human 0..0 growth hormone (hGH) as administered to humans) now con- °tains a peptide sequence which is unfamiliar to the reo a cipient. The result is predicatable. An immune response may be mounted to the unfamiliar sequence and a o e therapeutically important peptide now becomes an immunogen.

0 In addition to foreign proteins, mature native Soo proteins and bacterial proteins from other genera or species are also often incompletely processed. Examples "a 0 of this phenomenon include E. coli aspartate trans- 03 0 carbamylase (R-chain), E. coli tryptophan synthestase A protein, and E. coli bacteriophage T4 lysozyme.

(Fasman, Ed.. CRC Handbook of Biochemistry Molecular Biology. 111:308-313.) Others have attempted to resolve the N-terminal methionine problem and to produce N-terminal "Met-less" peptides or proteins in various ways. Baxter (U.S.

4,350,764) uses in vitro treatment with the protease -7 -3trypsin to cleave a precursor protein after protecting alternate cleavage sites. Fusion proteins have also been synthesized where the desired coding sequence is preceded by ATG, thus providing an "internal" methionine in the fusion cleavable by CNBr. Not only does this involve an extra preparation step, but has the more serious defect that the protein or peptide is also cleaved at any methionine residues in the remaining sequence.

EPO publication 127,305, published 5 December 1984, to Genentech discloses the production of Met-less hGH by employing a coding sequence which includes the native hGH leader peptide which apparently is workable in certain bacterial hosts to effect secretion of the resulting hGH. Gilbert 4,338,397) has employed the penicillinase leader sequence to effect the secretion of presumably N-terminal Met-less 1-globin. European Patent Application Serial No. 86302201.8, filed 25 March 1986, assigned to the same assignee and incorporated herein by reference, discloses the use of the leader sequence for bacterial phospholipase A (phoA) to effect secretion of certain, but not all, recombinant peptides.

None of the foregoing approaches provides a universal solution to the problem. Faced with the ne- .oo cessity to produce any particular recombinant protein in N-terminal Met-less form, the practitioner needs to seo lect from a repertoire of possibilities a procedure suitable for the particular peptide to be produced. The method of the invention described below expands this repertoire to provide still another pattern of applicauO *o 30 bility.

Disclosure of the Invention The invention furnishes a convenient enzyme for assuring the processing of N-terminal methionine -4residues from bacterially produced recombinant or other proteins. Also provided is the DNA encoding this enzyme permitting genetic manipulation of the recombinant host organism to effect the desired processing in vivo without the necessity of the separate step. The availability of the peptidase enzyme of the invention thus permits production in bacterial hosts of recombinant proteins which have reduced immunogenicity when used therapeutically.

In one aspect, the invention relates to a peptidase which cleaves N-terminal methonine residues from certain protein sequences--i.e., a methionine amino peptidase or N-terminal exopeptidase. The enzyme will be referred to herein as Met-aminopeptidase. The Metaminopeptidase enzyme includes proteins which have 1 activity of defined specificity (see below) and which immunoprecipitate with antibodies prepared against the protein of amino acid sequence shown in Figure 2 herein. The Met-aminopeptidase enzyme further includes proteins having this activity and which are encoded by DNA that hybridizes under specified conditions to the DNA illustrated in Figure 2 encoding the deduced amino 0° acid sequence. The invention also relates to antibodies Oo immunoreactive with protein of the amino acid sequence shown in Figure 2. including those raised by injection ao0° of this protein into a vertebrate.

In other aspects, the invention relates to a recombinant DNA sequence encoding the Met-aminopepti- S .0o dase. to plasmids bearing this sequence, and to e4 o o *o 30 microbial hosts transformed with these plamids, as well as to methods for producing N-terminal Met-less recombinant proteins in bacterial hosts or in vitro using the materials of the invention. In still another aspect, the invention relates to a method to obtain a 5 bacterial strain with high Met-aminopeptidase activity comprising screening generally peptidase-deficient (but not Met-aminopeptidase deficient) transformant hosts wherein the transformant has had introduced a portion of its own genome.

According to a first embodiment of this invention there is provided a method to obtain a DNA sequence encoding a bacterial Met- aminopeptidase, wherein said Met-aminopeptidase has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues, and does not cleave at other N-terminal residues, and wherein said Met-aminopeptidase releases methionine from a peptide selected from a first group; and a- releases no amino acids from a peptide selected from a second group; which method comprises: o preparing a plasmid-borne gene/library from a first bacterial strain; Stransformiing said gene library into a second bacterial strain that is S deficient in general peptidase activity; screening transformants for Met-aminopeptidase activity; and recovering plasmid DNA from transformants having said activity.

The first group consists of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; Met-Ala-Ser; Met-Gly-Gly; Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Thr-Gln-Leu; and S" Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys.

o The second group consists of: Met-Phe-Gly; Met-Phe-Ala-Gly; Met-Leu-Phe; Met-Met-Met; Leu-Leu-Leu; Leu-Gly-Gly; IUsy Met-Ala; Leu-Gly; Leu-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gln-Leu; FTMR/947 TMR/947u i 5a !t N-formyl-Met-Met-Met; Met-Phe; Met-Ser; Val-Gly-Gly; Thr-Gly-Gly; Trp-Gly-Gly; Phe-Gly-Gly; Met-Glu-His-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 -Gly; Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Gln-Leu-Cys; Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu; Thr-Val-Leu; Arg-Gly-Gly; S)2Ala-(Ala) -Ala; Ala-Ala-Ala; Glu-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and -Met-Arg-Phe acetate.

According to a second embodiment of this invention there is provided a method to obtain a DNA sequence encoding a bacterial Met- aminopeptidase, S wherein said Met-aminopeptidase has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues and wherein said Met- aminopeptidase S° releases methionine from a peptide selected from the first group; and releases no amino acids from a peptide selected from the second group; screening bacterial transformants for Met-aminopeptide activity, and recovering plasmid DNA from transformants having such activity; wherein the transformants were prepared by preparing a plasmid-borne gene library from a first bacterial strain; and transforming said gene library into a second bacterial strain that is deficient in general peptidase activity.

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5b According to a third embodiment of this invention there is provided a recombinant bacterium which contains an expression system functional in expression DNA encoding Met-aminopeptidase, wherein said Metaminopeptidase has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, wherein the Met-aminopeptidase releases methionine from a peptide selected from the first group; and releases no amino acids from peptides selected from the second group; an expression system functional in expressing the DNA encoding a Met-preceded desired recombinant foreign protein.

According to a fourth embodiment of this invention there is provided a method for producing an N-terminal Met-less recombinant protein in a bacterial host which method comprises: culturing a recombinant bacterium which contains an expression system Sfunctional in expressing DNA encoding Met-aminopeptidase- i effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, wherein the Met-aminopeptidase methionine releases methionine from a peptide selected from the first ~group; and releases no amino acids from a peptide selected from the second group; an expression system functional in expressing the DNA encoding a Met-preceded desired recombinant foreign protein, under conditions Sappropriate for the expression of said DNAs encoding said Met-aminopeptiduse and said desired recombinant foreign protein.

According to a fifth embodiment of this invention there is provided a method to prepare N-terminal methionine-free protein which comprises treating a Met-preceded prctein with an effective amount of Metaminopeptidase, wherein said Met-aminopeptidase is prepared by culturing transformant cells; which cells have been transformed with a recombinant DNA expression system comprising control sequences operably linked to DNA encoding Metaminopeptidase, wherein said Met-aminopeptidase has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and TMR/947u 1 5c does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the first group; and releases no amino acids from a peptide selected from the second group; said culturing under conditions which favor expression of said DNA encoding Met-aminopeptidase; and recovering Met-aminopeptidase from the transformants.

According to a sixth embodiment of this invention there is provided a Met-aminopeptidase in purified and isolated form characterized in that it has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the first group; and releases no amino acids from a peptide selected from second the second group.

According to a seventh embodiment of this invention there is provided an isolated DNA encoding an aminopeptidase wherein said Met-aminopeptidase has a specificity wherein it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the first group; and releases no amino acids from a peptide selected from the second group.

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44 4 44 O 4 i ji According to an eighth embodiment of this invention there is provided an expression system capable, when contained in a recombinant host, of expression a DNA encoding a Met-aminopeptidase which has a specificity wherein it effects cleavage of the N-terminal methionine residue from 04"4: Met-preceded peptides or proteins without cleavage of internal methionine S residues and does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the first group; and releases no amino acids from a peptide selected from the second group.

Rriof rrinfinin nf fhe nrawinns Figure 1 shows the N-terminal amino acid sequence protein of the Met-aminopeptidase of the invention.

Figure 2 shows 1.2 kb insert of pSYC1174 encoding peptidase illustrated in Figure 1.

Figure 2 shows an SDS gel of purified recombinant after processjigwjith the enzyme of the invention.

determined from the the Met-amino- IL-2 before and TMR/947u 5d Figure 4 shows the gene for ricin A.

j Modes of Carrying Out the Invention A. Definitions As used herein, "Met-aminopeptidase" refers to an enzyme which specifically cleaves the N-terminal methionine residue from a peptide sequence, and does not cleave at internal methionine residues or at N-terminal residues other than methionine. The Met-aminopeptidase of the invention appears to be specific for particular peptide sequences depending on the residue occupying position 2 and on the secondary or tertiary structure of the substrate protein or peptide. The precise specificity of the enzyme in this regard cannot b determined without testing nearly an infinite number of substrates: however, a useful rule of thumb is set forth by Sherman. et al, Bio Essays (1985) 3:27-31. Sherman et al based their considerations for specificity of Met-aminoi s o d y0 io i o j: 6 G 5 B TMR/947u Ci. i U~ peptidases on the observed forms of mutants of iso-l-cytochrome-C from yeast and the published primary sequence of 82 mature intracellular proteins. They conclude that methionine is usually cleaved from residues with a side chain having a radius of gyration of 1.2 A or less, but generally not cleaved from residues with side chains larger than 1.43 A. This is consistent with the observation that mutationally altered iso-1-cytochrome-C taken in consideration with other published sequences of other proteins from procaryotic and eucaryotic systems indicate that N-terminal methionine is cleaved when it precedes residues of alanine, cysteine, glycine, proline, serine, threonine, or valine, but not when it precedes residues of arginine, asparagine, aspartic acid, glutamine, glutamic acid, isoleucine, leucine, lysine, or methionine. These results are generally consistent with those set forth in the illustrations below. However, some exceptions occur where the radius of gyration for the second amino acid S" 20 is higher than 1.29 A and the secondary and tertiary structure or other conditions are particularly favorable. Therefore, this aspect of the specificity is intended as a general guideline, and it should be borne in 0o mind that even the specificity of the aminopeptidase 25 used to illustrate the present invention is not determined with exact precision, not all possible tertiary structures have been tested. Therefore, in order to fall within the definition of "Met-aminopeptidase", ooos the enzyme needs only to meet the requirement of specif- S 30 ic cleavage of N-terminal methionine without cleavage of internal methionine residues and without cleavage of N-terminal residues other than methionine from any peptide.

i -7- The preferred Met-aminopeptidases of the invention have N-terminal amino acid sequences substantially equivalent to that shown in Figure 1, and total amino acid sequences substantially equivalent to that encoded by the DNA illustrated in Figure 2. By "substantially equivalent" is meant that the protein retains the same activity in specifically cleaving N-terminal methionine residues from particular peptide or protein sequences with fundamentally the same underlying specificity with respect to secondary and tertiary structures or subsequent amino acid residues, even though minor alterations in amino acid sequence may be present. Such alteration, interchange, addition, or deletion of one or several amino acids in the sequence which do not appreciably alter activity do not remove a particular protein from this definition.

S0: For example, conservative amino acid substitu- SI. tions, such as substitution of a serine or an alanine 0 o residue for one or more of the cysteines at positions 45, 59, 78, 126, or 245, result in peptides which may 4retain the Met-aminopeptidase activity. In addition, there may be interchangeability of leucine, isoleucine, 0 and valine residues. Also, up to the first seven amino Sro acids at the N-terminus may be deleted, and portions of the downstream regions of the peptide beginning at amino acid 228 may not be essential for activity.

u Y a Of course, included as well are the neutral and salt forms )f the Met-aminopeptidases, as well as forms which contain additional non-protein moieties such as S 30 glycosylation, lipid residues, or acetylation.

"Peptidase-deficient" strain :efe s to a bacterial strain which is lacking in at least four peptidases other than Met-aminopeptidase which peptidases are normally found in the wild type.

i I- t;p -8o oa 40*0) 0 00 0o 0 0 4'' 0 0044L P 0 S 0 0 "N-terminal Met-less" protein, as used in this application, specifically refers to a protein lacking an N-terminal methionine, but which might include methionine residues elsewhere in its primary structure. The coding sequence for the protein will have an immediately preceding ATG start codon in reading frame. "N-terminal Met-less" is used as a convenient shorthand term so that the conditions surrounding this state need not be repetitively given. Specifically, "N-terminal- Met'-less" does not mean, in the context of this invention, that there are necessarily no methionine residues whatsoever in the protein sequence, nor is it intended to include proteins which had no possibility of an N-terminal methionine in the first place, such as those produced as fusion proteins or as secreted proteins, preceded before processing by a signal sequence. Thus, as used herein, "N-terminal Met-less protein" refers to a protein which is encoded by a DNA sequence wherein the mature protein is immediately preceded by an in-reading-frame ATG start codon and not part of a fusion to be subsequently cleaved by CNBr, trypsin, or other reagents. In the case of recombinant proteins, the constructions are clearly specified; for native or naturally recombined DNA sequences, the constructions may not be as easily 25 defined.

"Met-preceded protein" is a protein which contains an N-terminal methionine residue immediately preceding the first amino acid normally found in the particular mature protein.

30 "Cells", "cell cultures", "host cells", and the like refer to subject cells for recombinant DNA manipulations. As would be apparent from the context, these cells may be candidates for, or resultants of, transfer of new DNA sequences according to recombinant tech- -9niques. Techniques which are suitable for DNA uptake by cells include most prominantly. in vitro transformation. However other techniques such as transduction or conjugation may also be used. The definition further includes the progeny of the cells directly referred to.

It is understood that such progeny may not be precisely identical in DNA content to their parents, but such progeny are included in the definition so long as alterations due, for example, to accidental or -deliberate mutation do not destroy the ability of the cells to exhibit the properties conferred by the introduced DNA in a manner similar to that exhibited by tneir parents.

B. General Description The present invention achieves the production of N-terminal Met-less recombinant proteins in bacterial Shosts through the use of a Met-aminopeptidase. In the most preferred embodiment, the Met-aminopeptidase is S, generated at high levels in situ and processes the recombinant or other protein in vivo in the bacterial host. However, it is also possible to isolate or extract the desired recombinant or other protein from the Sshost cells and treat the extract in vitro with the Meta "o aminopeptidase obtained independently from a bacterial source.

"S With respect to the Met-aminopeptidase per se, :his enzyme has been produced and the DNA encoding it recovered by taking advantage of the ease in screening S E. coli strains which are generally peptidase deficient B 30 for enhanced production of the Met-aminopeptidase en- 0 0 coded in their own genome. In this process, a source of plasmid-borne and amplified DNA encoding Met-aminopeptidase is obtained, and the enzyme can then be prepared and purified directly from these cells. In addition

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co-transformation of recombinant hosts with this plasmid DNA. along with the expression vector for a desired recombinant protein, results in in situ production of the recombinant protein in N-terminal Met-less form.

A number of E. coli strains which are deficient in a multiplicity of peptidases ordinarily found in wild-type bacteria are known. For example. Miller, et al, J Bacteriol (1978) 135:603-611, discloses a number of bacterial strains which are pepti-dase deficient. One of these strains. CM89, which is deficient in peptidase N, peptidase A, peptidase B, peptidase D, and peptidase Q, was used in the illustration below.

However, other peptidase-deficient mutants of bacterial strains could be used as well.

Presumably, the genome in these strains still o contains the sequence encoding the Met-aminopeptidase activity, and the genomic DNA is therefore used to S construct a library by digestion with an appropriate Srestriction enzyme and cloning the fragments into carrier vectors. A variety of such carrier vectors is available, including the pUC series and pBR322. Plasmid DNA may then, if desired, be amplified using any convenient wild-type host before isolation of the plasmid DNA Do and transformation back into the peptidase-deficient strain for screening.

o'"a The transformed peptidase-deficient bacteria are then screened for production of the desired Metaminopeptidase by assaying crude extracts for their ability to cleave an appropriate substrate. A strain which shows an elevated level of Met-aminopeptidase is then conveniently used as a source for this enzyme or as a source of plasmid DNA for co-transformation with the expression vector for a recombinant protein.

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-11- In addition the plasmid DNA from this strain can be used to probe the genome of wild-type bacteria for the appropriate Met-amino-peptidase encoding sequences. Suitable stringencies are those characteristic of the hybridization conditions described specifically hereinbelow. These particular conditions need not be used, but those having the homology requirements. These retrieved sequences are also, of course, capable of being expressed, either under control of -their own promoters, or using other promoters known in the art, such as the trp or penicillinase promoters.

The Met-aminopeptidase protein produced herein is purified and the purified protein used to obtain *to antibodies using suitable immunization protocols. The 15 purification is conducted by disrupting the cells and isolating the enzyme from the supernatant lysate. This isolation may conveniently include treatment with an anion exchange resin under conditions wherein the ,I protein is adsorbed, followed by elution in appropriate buffer. Suitable anion exchange resins include DEAE I conjugated to various carbohydrate supports. Other anion exchange resins, well known in the art, may also o 0 S° *be used.

Antibodies raised in response to the purified 25 protein in rabbits, rats, or other mammals are useful in identifying Met-aminopeptidase proteins from a variety of microorganisms.

Large numbers of recombinant proteins are candidates for production as mature proteins in processed form, free of N-terminal methionine, using the method of the invention. For example, lymphokines such as IL-2, IL-1; the a- and y-interferons (i-interferon normally contains an N-terminal methionine in its mature form); tumor necrosis factor; and other proteins associ-

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-r I i -12ated with the lymphatic systems are thus produced.

Also, various hormones, such as growth hormones, insulin, ACTH, endorphins, and other peptide hormones can be produced recombinantly. Other candidates for recombinant production include enzymes such as tissue plasminogen activator, urokinase, and enzymes useful in industrial applications such as alcohol dehydrogenase. Other proteins include toxins such as diphtheria and ricin toxin and various factors such as epidemal growth factor and transforming growth factor. The foregoing are merely exemplary, and, in principle, any desired protein, once its gene is obtained, can be expressed as a mature protein by linking it in reading frame to an immediately upstream ATG start codon and providing the necessary control sequences. The method of the invention permits oso any of these proteins to be conveniently produced with- 1 out N-terminal methionine.

SAs stated above, the Met-aminopeptidase may be used in two general ways. The enzyme may be isolated, for example, from the specific cells producing it in relatively large quantity from plasmid-borne DNA, and added to an in vitro reaction mixture to effect N-terminal methionine processing, or the Met-aminopeptidase encoding plasmids may be cotransformed along 25 with expression vectors for a desired protein into a recombinant bacterial host LO permit in vivo processing.

In the in vitro approach, the purified Metaminopeptidase is added to a reaction mixture containing I unprocessed protein and suitable salt and buffer. The reaction mixture is incubated at a temperature of preferably about 30 0 C overnight to permit the processing to occur. The enzyme exhibits a requirement for cobalt ion. A typical reaction mixture might contain about 1 mg/ml substrate protein, about 80 ug/ml of enzyme in i 4 -13pH 7-8 phosphate buffer and about 0.2 mM cobalt ion.

The foregoing typical mixture is, of course, merely illustrative and the concentrations of the components can be varied in a continuum depending on the nature of the substrate and the time and temperature conditions employed. Complete processing can be verified by measuring the amount of methionine residue released, by comparing the mobility on SDS PAGE of the processed and unprocessed subject protein, or by sequencing the substrate material contained in the mixture.

In the in vivo approach, plasmid DNA is isolated from the Met-aminopeptidase source strain and used to transform cells which already harbor or which are con- Scomitantly or subsequently transformed to harbor an ex- S 15 pression system for the proteins. When used in bacterial sources for bacterial enzymes, the unprocessed substrates may be produced as a part of the complement of proteins ordinarily generated by the microorganism.

More commonly, the peptidase generated in situ is used to process recombinantly produced proteins and the cells must be at some point transformed to contain the expression system for the desired protein.

C. Standard Techniques 25 Standard methods for transformation of bacteria, selection of successful transformants using markers, preparation of plasmid vectors, and screening of gene or cDNA bahks are now well understood in the art.

S•"S For convenience, a selection of procedures particularly useful in the example set forth below are presented here. Most such methods, or alternative workable ones, are found in Maniatis, et al, Molecular Cloning A Laboratory Manual (1982). Cold Spring Harbor Press.

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i r~ll IPI-rrPILZi=U" -14o o 0 0 f ftD Of ftf .l ftf Sof ft *0400ts ft ft C.1. Hosts and Control Sequences The cells suitable for cotransformation with vectors bearing Met-aminopeptidase and expression systems for protein are bacterial. Most frequently the hosts are various strains of E. coli. However, other microbial strains may also be used, such as bacilli, for example Bacillus subtilis, various species of Pseudomonas, or other bacterial strains. In such procaryotic systems, plasmid vectors which contain replication sites and control sequences derived from a species compatible with the host are used. For example, E. coli is typically transformed using derivatives of pBR322, a plasmid derived from an E. coli species by Bolivar, et al, Gene (1977) 2:95. pBR322 contains genes for ampicillin and tetracycline resistance, and thus provides additional markers which can be either retained or destroyed in constructing the desired vector.

Commonly used procaryotic control sequences which are defined herein to include promoters for transcription initiation, optionally with an operator, along with ribosome binding site sequences, include such commonly used promoters as the beta-lactamase (penicillinase) and lactose (lac) promoter systems (Chang, et al, Nature (1977) 198:1056) and the tryptophan (trp) promoter system 25 (Goeddel, et al Nucleic Acids Res (1980) 8:4057) and the lamDda &erived PL promoter and N-gene ribosome binding site (Shimatake, et al, Nature (1981) 292:128), which has been made useful as a portable control cassette, as set forth in copending Application Serial No. 578,133, filed February 8, 1984, and assigned to the same assignee. However, any available promoter system compatible with procaryotes can be used.

C.2. Transformations The cells are transformed using calcium treatment employing calcium chloride, as described by Cohen.

Proc Natl Acad Sci (USA) -(1972) 69:2110. or the 2method described in Maniatis, et al. (supra).

C.3. Vector Construction Construction of suitable vectors containing the desired coding and control sequences employs standard ligation and restriction techniques which are well understood in the art. Isolated plasmids, DNA sequences, or synthesized o ligonuc leot ides are cleaved, tailored, and religated in the form desired.

Site specific DNA cleavage is performed by treating with the suitable restriction enzyme (or enzymes) under conditions which are generally understood in the art, and the particulars of which are specified by the manufacturer of these commercially available restriction enzymes. See, New England Biolabs, Product Catalog. In general, about 1 jig of plasmid or DNA sequence is cleaved by one unit of enzyme in about jil of buffer solution; in the examples herein, typically, an excess of restriction enzyme is used to insure complete digestion of the DNA substrate. Incubation times of about one hour to two hours at about 37 0

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are workable, although variations can be tolerated.

After each incubation, protein is removed by extraction with phenol/chloroform, and may be followed by ether o extraction, and the nucleic acid recovered from aqueous fractions by precipitation with ethanol followed by running over a Sephadex G-50 spin column. If desired, size separation of the cleaved fragments may be performed by polyacylamide gel or agarose gel electrophoresis using standard techniques. A general description of 3 -16o 04* o 4,0 44 0 0 0444 *c4~4 40o size separations is found in Methods in Enzymology (1980) 65:499-560.

Restriction cleaved fragments may be blunt ended by treating with the large fragment of E. coli DNA polymerase I (Klenow) in the presence of the four deoxynucleotide triphosphates (dNTPs) using incubation times of about 15 to 25 min at 20 to 25 0 C in 50 mM Tris pH 7.6. 50 mM NaCl. 6 mM MgCl 6 mM DTT and 5-10 yM dNTPs. The Klenow fragment fills in at 5' sticky ends but chews back protruding 3' single strands, even though the four dNTPs are present. If desired, selective repair can be performed by supplying only one of the, or selected, dNTPs within the limitations dictated by the nature of the sticky ends. After treatment with Klenow, the mixture is extracted with phenol/chloroform and ethanol precipitated followed by running over a Sephadex G-50 spin column. Treatment under appropriate conditions with Sl nuclease results in hydrolysis of any single-stranded portion.

Synthetic oligonucleotides are prepared by the triester method of Matteucci, et al (J Am Chem Soc (1981) 103:3185) or using commercially available automated oligonucleotide synthesizers. Kinasing of single strands prior to annealing or for labeling is achieved 25 using an excess, apprc'imately 10 units of polynucleotide kinase to 0.1 nmo'l substrate in the presence of 50 mM Tris, pH 7.6, 10 iiM MgCl 2 5 mM dithiothreitol, 1-2 mM ATP. 1.7 pmoles y32P-ATP (2.9 mCi/mmole), 0.1 mM spermidine, 0.1 mM EDTA.

Ligations are performed in 15-30 p.l volumes under the following standard conditions and temperatures: 20 mM Tris-Cl pH 7.5. 10 mM MgCl2. 10 mM DTT.

33 jig/ml BSA. 10 mM-50 mM NaCl, and either 40 jiM ATP. 0.01-0.02 (Weiss) units T4 DNA ligase at 14 0 C (for -17- 4.

04 4, 4 I 4 44 4 o C~C, o 4* 0 0 4 0040 ,3~ 4 0 4 0004 4 44 4 4 "sticky end" ligation) or 1 mM ATP. 0.3-0.6 (Weiss) units T4 DNA ligase at 14°C (for "blunt end" ligation).

Intermolecular "sticky end" ligations are usually performed at 33-100 jig/ml total DNA concentrations (5-100 nM total end concentration). Intermolecular blunt end ligations (usually employing a 10-30 .fold molar excess of linkers) are performed at 1 -iM total ends concentration.

In vector construction employing "vector fragments", the vector fragment is commonly treated with bacterial alkaline phosphatase (BAP) in order to remove the 5' phosphate and prevent religation of the vector.

BAP digestions are conducted at pH 8 in approximately 150 mM Tris, in the presence of Na+ and Mg 2 using about 1 unit of BAP per .ig of vector at 60°C for about one hour. In order to recover the nucleic acid fragments, the preparation is extracted with phenol/chloroform and ethanol precipitated and desalted by application to a Sephadex G-50 spin column. Alternatively, religation can be prevented in vectors which have been double digested by additional restriction enzyme digestion of the unwanted fragments.

For portions of vectors derived from cDNA or genomic DNA which require sequence modifications, site specific primer directed mutagenesis is used according to the method of Zoller, et al, Nucleic Acids Res (1982) 10: 6487-6500. This is conducted using a primer synthetic oligonucleotide complementary to a single stranded phage DNA to be mutagenized except for limited mismatching, representing the desired mutation. Briefly, the synthetic oligonucleotide is used as a primer to direct synthesis of a strand complementary to the phage, and the resulting double-stranded DNA is transformed into a phage-supporting host bacterium. Cultures of the -18transformed bacteria are plated in top agar, permitting plaque formation from single cells which harbor the phage.

Theiratically, 50% of the new plaques will contain the phage having, as a single strand, the mutated form: 50% will have the original sequence. The resulting plaques are hybridized with kinased synthetic primer at a temperature which permits hybridization of an exact match, but at which the mismatches with the original strand are sufficient to prevent hybridization. Plaques which hybridize with the probe are then picked, cultured, and the DNA recovered. Details of site specific mutation procedures are described below in specific examples.

S C.4. Verification of Construction Correct ligations for plasmid construction are confirmed by first transforming E. coli strain MM294 obtained from E. coli Genetic Stock Center, CGSC 46135, or other suitable host with the ligation mixture. Suco a cessful transformants are selected by ampicillin, tetraon cycline or other antibiotic resistance or using other markers depending on the mode of plasmid construction, °OQ as is understood in the art. Plasmids from the transformants are then prepared according to the method of Clewell, D. et al, Proc Natl Acad Sci (USA) (1969) o 62:1159, optionally following chloramphenicol amplification (Clewell, D. J Bacteriol (1972) 110:667).

The isolated DNA is analyzed by restriction and/or sequenced by the dideoxy method of Sanger, et al, Proc Natl Acad Sci (USA) (1977) 74:5463 as further described by Messing, et al, Nucleic Acids Res (1981) 9:309, or by the method of Maxam, et al, Methods in Enzymoloqy (1980) 65:499.

-19- Hosts Exemplified Host strains used in cloning and expression herein are as follows: For cloning and sequencing. and for expression of construction under control of most bacterial promoters, E. coli strain MM294 (supra), Talmadge. et al.

Gene (1980) 12:235: Meselson, et al, Nature (1968) 217:1110. was used as the host. For expression under control of the PLNRBS promoter. E. coli &train K12 MC1000 lambda lysogen. N7 N 53cI8575usP 8 0, ATCC 39531 (hereinafter sometimes referred to as MC1000-39531) is used. To verify the presence of an insert, strains complementing the characteristic of the backbone vector in the region of the insert are used.

For example, for the pUC series, E. coli strain DG99, o which produces blue colonies on X-gal indicator medium in the absence of insert and white colonies in the presence of insert is used.

D. Examples 0 04o The following examples are intended to illuso trate, but not to limit, the invention.

044 Preparation of a Source for Plasmid Met- Aminopeptidase Encoding DNA Chromosomal DNA was extracted from E. coli o oStrain CM89 (supra) by the method of Silhavy, et :al. Experiments with Gene Fusions (1984), Cold Spring Harbor Laboratory, New York, 137-139, and stored in mM Tris, pH 8.0. 1 mM EDTA (TE) buffer. The DNA was digested with Sau3AI at 0.1 U/jig and 0.2 U/jig for 1 hr at 37 0 C. After reaction termination and ethanol precipitation. the partially digested DNAs were pooled and fractionated on a 10-40% sucrose gradient using a

I

Beckmann SW28 rotor at 26.000 rpm for 24 hr at 15 0

C.

Fractions containing 4-8 kb fragments were pooled, purified on a DE52 column, ethanol precipitated from the eluant and stored in TE buffer.

A 4 ig portion of the chromosomal DNA was then ligated with 0.5 g of BamHI-digested, BAPtreated pUC18 vector fragments. The ligation mixture was used to transform E. coli DG99 and plated on lactose indicator plates to confirm the presence of inserts in the plasmids. Approximately 94% of the transformants indeed contained DNA inserts of approximately 4 kb.

Therefore, 18 1il of the ligation mixture was used to transform E. coli MM294 to Amp R to obtain the gene library. Successful transformants were picked and S 15 used to inoculate 700 ml of ampicillin-containing culture medium for plasmid DNA preparation.

Plasmid DNA was obtained from the cells as described in C.4 (Clewell, Proc Natl Acad Sci (USA) (1969)) above and used to transform E. coli CM89. Successful transformants selected for Amp were plated Sinto microtiter trays for screening and approximately 1,000 colonies were screened.

Single colonies were picked into 200 Li minimal medium (see, for example, U.S. Patent 4,518,584, incorporated herein by reference) supplemented 5% v/v each with 2X L-Broth (DIFCO) plus 1% NaC1, 10% Casamino o" acids, and 10X yeast nitrogen base. After overnight growth at 37 0 C, cells were washed twice in 0.1 M Tris*HC1 pH 7.4. The cells were lysed by adding v1 of a 1 mg/ml lysozyme solution in the same buffer, followed by 3 cycles of freeze-thaw. Then 180 il 0.1 M potassium phosphate buffer (KPO pH 7.4 0.2 mM CoC12, containing 72 .g Met-Gly-Met-Met, 36 Lg L-amino acid oxidase, 4-5 ±g horseradish peroxidase.

i i ililil -21and 18 ig O-dianisidine dihydrochloride was added to each well; color formation was evident in Met-aminopeptidase-containing lysates. Of the approximately 1000 colonies screened, 10 showed increased rate of release of Met from Met-Gly-Met-Met, and were further screened for failure to release Leu from Leu-Gly-Gly under the same conditions. One successful colony was designated pSYC1174. E. coli pSYC1174 was deposited with the American Type Culture Collection 27 August 1985 and has accession number 53245.

D.2. Recovery of the Met-Aminopeptidase Coding Sequence The E. coli strain harboring pSYC1174 (also designated 18E7) gave approximately one-hundred-fold 15 higher activity in the Met-Gly-Met-Met substratemediated in vitro assay, conducted generally as described above.

S* Plasmid DNA was isolated from strain 18E7 and its the Met-aminopeptidase-encoding plasmid pSYC1174 was isolated. pSYC1174 carried an insert of 3.2 kb in the S"pUC18 vector at the BamHI site. A 1.2 kb fragment was ,o excised from the 5' end of the insert by EcoRI/Clal digestion and inserted into pUC18 and pUC19: pSYC1174 So was digested with ClaI, blunted with Klenow and then with EcoRI to excise the 1.2 kb EcoRI/blunt fragment.

This fragment was inserted into EcoRI/SmaI-digested o pUC18 or pUC19, which results in opposite orientation to the lac promoter on the host plasmids. Both of the resulting vectors pSYC1187 and pSYC1188, when transfected into CM89, showed levels of amino peptidase production comparable to that shown by pSYC1174. These results indicate that both the Met-aminopeptidase gene and its promoter are located within the 1.2 kb fragment.

II- -22- Figure 2 shows the complete nucleotide sequence of the 1.2 kb fragment determined by dideoxy sequencing. The open reading frame starting with ATG is at positions 219-1010 and encodes a putative protein of 264 amino acids having a calculated molecular weight of 29,333. The first 64 amino acids deduced correspond to those obtained using amino acid sequencing of the purified protein as described in D.3 below. The location of two tandem promoters associated with this open reading frame is also shown and are labeled P1 and P2. (The numbers in the lefthand column represent nucleotides, those in the righthand column, amino acids.) The 1.2 kb fragment above was used to probe the foQo genomic DNA of E. coli by Southern blot and hybridized 15 to bands of 3.6, 5.2. and 1.35 kb that were generated by digestion with PstI, EcoRI, and BssHII, respectively, but not to other regions of the chromosome, thus indicating that the gene is present as a single copy in E.

S' coli. Evaluation of the sequence at the 3' end of the gene also leads to the conclusion that are probably no o cotranscribed genes downstream from the Met-aminopeptidase. Evaluation of the sequence at the 5' end indicates the presence of tandem promoters, as shown.

oo ~The nucleotide sequence shown in Figure 2 that encodes the deduced amino acid sequence 1-264 (or its complement) is generally useful to probe genomic microbial DNA for additional Met-aminopeptidase encoding sequences. Thus, this insert is a convenient tool to obtain this desired DNA from, for example, Bacillus subtilis, Pseudomonas, or yeast. Appropriate stringency is that associated with hybridization in a buffer containing 6 x SSC, 0.01 M EDTA, 5 x Denhardt's, SDS at 65 0 C for sufficient time to complete reaction, followed by washing with 3 x SSC at 65°C. That is, DNA 'r

I

-23which hybridizes to the above nick-translated probe under these conditions and which encodes protein having Met-aminopeptidase activity as herein defined, is included within the invention, and encodes Met-aminopeptidase protein within the invention.

D.3. Characteristics of Met-Aminopeptidase from E. coli pSYC1174 The Met-aminopeptidase was purified from crude extracts of E. coli pSYC1174 and the purified protein was analyzed for ability to release amino acids using a variety of peptide substrates.

For purification, overnight cultures of E. coli SYC1174 in Brain Heart Infusion broth were washed twice 15 in KPO buffer (20 mM. pH 7.4) with 0.2 mM CoCl 2 4 2 and sonicated. PMSF (0.1 mM) was added to the sonicate. The sonicate was centrifuged, and the supernatant passed over DEAE-Sepharose Fast Flow. The enzyme was eluted with a NaC1 gradient, 0-0.25 M, in the same buffer. Fractions with Met-aminopeptidase activity were S.1 pooled, concentrated using 30.000 MW Centricon filters, 0 444 and passed over an S-200 Sephacryl column, in the same o" buffer plus 1 mM methionine. Active fractions were pooled and concentrated as before.

The subunit molecular weight was determined to be approximately 32,000 by reducing SDS PAGE (Laemmli, J oou <Mol Biol (1973) 80:575-599), and enzyme purity was estimated to be 95%. The protein is thus of approximately S° the predicted size for a 264 amino acid protein. Estimates of quantity based on densitometry of the stained gel showed the Met-aminopeptidase to be about 15-20% of cellular protein.

i -24- N-terminal sequencing was performed on the purified peptidase. Results for the first 65 amino acids are given in Figure 1.

Purified Met-aminopeptidase was analyzed for the ability to release amino acids from a variety of peptide substrates, using a modified L-amino acid oxidase-HRP-ODAD assay, generally as described above and TLC method. For the first mentioned assay, 10 iLi of the protein solution, in this case the lysate.-was' added to 90 il of substrate solution containing 4 mM Met- Gly-Met-Met, 0.1 M potassium phosphate buffer, pH and 0.2 mM CoC12. The tubes containing the reaction mixtures were incubated at 30 0 C for 10 min and the reac- 0o09 tion was stopped by placing the tubes in a boiling water 15 bath for 2 min. After the addition of 0.9 ml color development mixture (0.1 M Tris HC1, pH 7.4, containing S0.2 mg L-amino acid oxidase, 0.03 mg horseradish peroxidase, and 0.2 mg O-dianisidine dihydrochloride), the a oi tubes were incubated for 30-60 min at 30 0 C and the optical density read at 440 nm.

o, The TLC method used silica gel plates with a o solvent mixture of n-butanol-acetic acid-water (120:50:30 Amino acids released were detected and identified after spraying the plates with ninhydrin reagent.

Methionine was released from the following peptides: Met-Ala-Met: Met-Gly-Met-Met: Met-Gly-Met; Met-Ala-Ser; Met-Gly-Gly; Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys- Thr-Gln-Leu; and Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln- Leu-Cys.

No amino acids were released from: Met-Phe-Gly; Met-Phe-Ala-Gly; Met-Leu-Phe; Met-Met-Met; Lt:u-Leu-Leu: Leu-Gly-Gly: Met-Ala: Leu-Gly; Leu-Ala-Pro-Thr-Setr-Ser-Ser-Thr-Lys-Lys- Thr-Gln-Leu; N-tormyl-Met-Met-Met: Met-Phe: Met-Ser; ~Val-Gly-Gly; Thr-Gly-Gly; Alit Trp-Gly-Gly; Phe-Gly-Gly; Met-Glu-His-Phe-Arg-Try-Gly; Met-Lys-Airg-Pro-Pro-Gly-Phe-Ser-Pro- Phe-Arg: 4 dy- (Gly) 3 -Gly; Phe-Gly-Gly; Ser-Ser-Ser; a Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln- Leu-Cys: Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys- Gln-Leu: Thr-Val-Leu: Arg-Gly-Gly; Ala- (Ala) 2 -Ala: Ala-Ala-Ala; -26- Glu-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly: Ile-Gly-Gly: Met-Arg-Phe acetate.

The peptidase activity was completely inhibited by 1 mM EDTA and requires about 1-200 mM phosphate ion and 0.02-2.0 mM Co for maximum activity.

+2 +2 Co could not be substituted for- by Mn Cu 2 Zn 2 or Mg 2 ions. The activity was also severely reduced when Tris was substituted for potassium phosphate buffer, but this activity can be restored by addition of sodium or potassium salts.

From the foregoing results, it is clear that the peptidase cleaves only N-terminal methionine and has other specificity requirements as well. The nature of the second and third amino acid in sequence appears to be significant, and a minimum of three amino acids in the peptide appears to be required. The results on short chain peptides may not, however, be completely determinative in terms of the requirements for succeedo ing amino acids, as folding in larger proteins may provide secondary and tertiary structures which alter the specificity as regards residues 2 and 3. In addition, the specificity is dependent on conditions, and peptides which fail to undergo hydrolysis under the specific *l conditions used may yet be hydrolyzed if the conditions are altered.

While in general Met-aminopeptidase cleaves N-terminal methionine when the second residue has a side chain with a radius of gyration smaller than 1.29 A, and while it is generally expected that cleavage will not occur when the side-chain size is larger than 1.43 A, exceptions do occur, notably that of the ricin A

S_

i, -27described below, wherein the radius of gyration for lie, the second amino acid, is 1.56 A. Thus, the effects of neighboring amino acids and the secondary and tertiary structure of the substrate also appear to have an impact on the specificity.

In addition, the Met-aminopeptidase purified from pSYC1174 as above was injected into rabbits using standard protocols and adjuvants, to obtain antisera specifically reactive with Met-aminopeptidase protein.

D.4. Preparation of N-Terminal Met-less IL-2 E. coli MM294 carrying pSYC1143. an expression vector for a recombinant IL-2 mutein with the N-terminal K"d sequence in the mature protein: Ala-Pro-Thr-Ser, under 15 the control of the trp promoter was transformed with plasmid DNA (designated pSYC1174) prepared from E. coli pSYC1174. Successful transformants were selected by R R SAmp and Tet

R

showing the presence of both desired plasmids.

Cells containing both plasmids were grown overnight at 37 0 C in minimal medium plus tryptophan O. mg/1, casamino acids 5 g/l, and both ampicillin 50 mg/l and tetracycline 5 mg/l. The culture was then washed Sand resuspended in the same medium minus tryptophan, in order to de-repress IL-2 synthesis, and incubated at 37 0 C for 4 hr.

The IL-2 thus produced is contained in intracellular refractile bodies. The refractile bodies were purified by repeated sonication and washing in 8 mM EDTA and finally resuspended in 5% SDS. The IL-2 was further purified by HPLC, using a Vydac C4 reverse phase column and a gradient of water to acetonitrile in 0.1% trifluoroacetic acid. The N-terminal sequence was deter- -28mined for the purified IL-2, and showed the following mixture: Met-Ala-Pro- 0- Ala-Pro- 25-30% Pro- 70-75% Control cultures grown and induced as above, but containing only pSYC1143 gave produced IL-2 wherein the purified protein has the composition 70% Met-Ala-Pro and 30% Ala-Pro.

(pSYC1143 contains the IL-2 sequences under the control of the trp promoter and the cry positive retroregulator sequence. It is prepared from pFC51.T, which contains this expression system as a 0.95 kb EcoRI fragment, and pACYC184, which is a host vector compatible "i

R

15 with pUC18 carrying a Cm marker. The expression system is prepared as an EcoRI digest of pFC51.T and ligated into EcoRI-digested pACYC184 to obtain pSYC1143. pFC51.T is extensively described in European Patent Application Serial No. 85306183.6, filed August 1985, assigned to the same assignee and incorporated herein by reference.) Q 09 In Vitro Processing of Met-IL-2 L's a l The purified Met-aminopeptidase was also used to process the purified IL-2 in vitro. The reaction mixture contained 50 pil of stock solution containing o o 1.7 mg/ml of IL-2 prepared above in 0.05% SDS; 40 -il of 0.1 M potassium phosphate buffer, pH 7.5 containing 0.2 mM CoCI12 and 10 1il of a 1:10 dilution of Metaminopeptidase purified from E. coli pSYC1174 stock containing 8 mg/ml. The reaction mixture was incubated at 300 overnight and the degree of processing assessed usi g SDS PAGE and N-terminal sequencing. Figure 3 shows the results of SDS PAGE performed on the unreacted -29-

J

a o 4444 e So 3 0 0 a o o 4 0 4444 IL-2 and IL-2 in the presence of enzyme. After incubation, the presence of a slightly smaller molecular weight protein replaces the band shown by the original Met-preceded protein. The N-terminal sequence for the purified IL-2 before enzyme treatment was 74% Met-Ala- Pro- and 26% Ala-Pro: after enzyme treatment, it was 94% Ala-Pro- and 6% Met-Ala-Pro.

D.6. Construction of Ricin A Expression Vector-s A host vector for the ricn A sequences, pSYC1089, which contains the phoA promoter, leader and coding sequence with a modification to provide a NarI site at the C-terminal end of the leader sequence, followed by the B. thuringiensis positive retroregulator was constructed as follows.

pSYC997: PhoA Promoter and Leader, Modified to Contain NarI Site Plasmid pEG247, a 25 kb plasmid containing the 20 2.6 kb phoA structural gene as a HindIII/XhoI fragment was used as a source of the phoA gene. This plasmid was obtained from M. Casadaban and was constructed in a manner analogous to that set forth in Groisman, E. A., et al, Proc Natl Acad Sci (USA) (1984) 81:1840-1843.

25 Indeed, by applying the procedures set forth in the foregoing reference, the phoA gene may be conveniently cloned into any desirable backbone vector.

The HindIII/XhoI 2.6 kb fragment from pEG247 was purified and cloned into pUCIB, a 2.7 kb plasmid containing an ampicillin resistance marker and a polylinker permitting convenient insertion of desired sequences. pUC18 was digested with HindIII/SalI, and the linear vector ligated with the isolated phoA fragment. The ligation mixture was used to transform E.

T

coli DG99, a strain comparable to E. coli JM103 or JM105, to Amp and the construction of the intermediate plasmid pSYC991 in successful transformants.

which had been screened for inserts into pUC18, was verified.

pSYC997 which contains the desired Narl modification was prepared from pSYC991 by site-directed mutagenesis. The PvuII/PvuII 770 base pair fragment was obtained from pSYC991. It includes a porti-on of the phoA promoter and the upstream N-terminal sequences of the mature alkaline phosphatase, and thus, also, the entire leader sequence. This fragment was ligated into the Smal site of M13mpll and single stranded phage was prepared as template for the mutagenesis. In the muta- S 15 genesis, the synthetic 26-mer, 5'-TTCTGGTGTCGGCGCCTTTGTCACAG-3' 0 (the superscript line shows the Narl site) was used as primer and probe. The mutagenized phage particles were t 20 then used to prepare RF-DNA as a source for the desired leader sequence containing the Narl site.

SpSYC1015: Cm- Marker Backbone Vector pSYC1015, which provides chloramphenicol resiso tance, a replicon, and suitable restriction sites in the phoA gene, is also constructed from pSYC991. pSYC991 was first digested with HindIII/BamHI, and the approximately 2.6 kb fragment containing the phoA gene was purified and ligated with the purified 3.65 kb vector 30 fragment from HindlII/BamHI-digested pACYC184. pACYC184 is available from ATCC and contains the chloramphenicol gene (Cm a bacterial replicon, and HindIII and BamHI sites in the tetracycline resistance gene. The i i -31- 0 tf

(I

II',

4 4 o o 4 4 9 ligation mixture was used to transform E. coli MM294 to

R

Cm and the construction of pSYC1015 was verified by restriction analysis and sequencing.

Additional phoA-Containing Intermediates Two additional intermediate plasmids, pSYC1052 and pSYC1078. were constructed in order to provide a suitable host vector for the B. thuringiensis positive retroregulator.

pSYC1052 was constructed by ligating the purified small HindIII/BssHII fragment containing the phoA promoter and Narl site from modified leader pSYC997 into HindIII/BssHII-digested pSYC1015, which has, thus, the unmodified phoA sequences deleted. The resulting vector pSYC1052 was confirmed in E. coli transformants

R

to Cm pSYC1078 is a modified form of pSYC1052 with the BamHI site in front of the phoA promoter deleted.

In order to delete this BamHI site, pSYC1052 was sub- 20 jected to partial BamHI digestion, filled in using DNA polymerase I (Klenow) in the presence of the four dNTPs, and religated under blunt-end conditions. The desired resulting plasmid, now containing a unique BamHI site just 3' of the phoA gene, was confirmed after screening 25 successful Cm R transformants.

pHCW701: Source of the Retrorequlator The ability of the 3' sequences of the gene encoding crystal protein from B. thurinqiensis (the cry 30 gene) to enhance the expression of upstream coding sequences was described and claimed in copending U.S.

Patent Application 646,584. filed 31 August 1984. assigned to the same assignee and incorporated herein by reference. Briefly, these sequences are characterized 0.104 0)

I,

__1 l _rn -32by a DNA sequence which transcribes to a corresponding RNA transcript capable of forming a stem and loop structure having a cytosine-guanine residue content of about 43%. When ligated about 30-300 nucleotides from the 3' end of the gene, a positive retroregulatory effect is shown on the gene expression. The positive retroregulator was prepared as a 400 bp EcoRI/BamHI restriction fragment, which was blunt-ended and ligated into pLW1, an expression vector for interleukin-2.

(pLW1 is a pRBR322 derivative containing a replicon effective in E. coli, a Tet R gene, the E.

coli trp promoter, ribosome binding fragment and a 706 bp HindIII/PstI DNA fragment which includes the gene for human IL-2. pLW1 has been deposited with ATCC under the terms of the Budapest Treaty and has accession no.

39405.) pHCW701 was completed by blunt-ending the 400 bp EcoRI/BamHI fragment containing the positive retroregulator of the cry gene with Klenow and the four 20 dNTPs, and ligating the blunt-ended fragment using T4 ligase and ATP into Stul-digested plasmid pLWI. Two possible orientations of insert can result, which are °o00 easily distinguishable by restriction analysis. The o desired plasmid, designated pHCW701, has the recreated BamHI site closer to the 3' end of the IL-2 gene. This plasmid was deposited with ATCC under the terms of the Budapest Treaty and has accession no. 39757.

Completion of pSYC1089 30 To complete pSYC1089, pHCW701 was digested with EcoRI, filled in using Klenow and the four dNTPs, then digested with BamHI. and the 400 bp fragment containing the positive retroregulator recovered. pSYC1078 was digested with Aval, filled in with Klenow and the four -33dNTPs, and then digested with BamHI. The ligation mixture was transformed into E. coli MM294 and the construction of the desired plasmid pSYC1089, a 5.5 kb

R

plasmid conferring Cm was confirmed. pSYC1089 contains the sequences for the phoA promoter and leader (with Narl site) sequence and structural gene immediately upstream of a BamHI site, followed by the positive retroregulator sequences of the cry gene.

Ricin A The ricin A coding sequences were obtained from pRA123, more specifically, an M13 subclone of pRA123, described below, through construction of pRAT1. pRA123 was deposited with ATCC 17 August 1984 and has accession no. 39799. The construction of pRATI from pRA123 is described extensively in U.S. Serial No. 653,515 filed September 1984, assigned to the herein assignee and incorporated herein by reference. Briefly, pRA123, which contains the entire ricin A coding sequence (see Figure was modified to provide this sequence as a HindIII/BamHI cassette with a termination codon in the proper position after amino acid 265, and with a start codon in position immediately preceding the mature sequence. pRA123 was digested with BamHI and the approximately 896 bp BamHI/BamHI fragment was isolated and subcloned into M13mpl8 in an anti-sense orientation relative to the lac promoter in the M13 vector. The phage single stranded DNA was subjected to two stages of 0 primer directed mutagenesis using as primers, the 30 sequence: 5'-CACAGTTTTAATTGCTTATAAGG-3'.

-34which places the TAA termination codon in proper reading frame at the terminus of the ser-gln-phe C-terminus of the ricin A chain followed by: 5'-CTTTCACATTAGAGAAGCTTATGATATTCCCCAAAC-3', which places the desired HindIII/ATG start codon diad immediately upstream of the N-terminal ile-phe-pro-lys sequence of ricin A. The modified phage were identified after each mutagenesis using the appropriate above primers as probes. The desired constructs were then double digested with HindIII and BamHI and the appropriate ricin A coding fragment isolated. pRATI was completed by ligation of the HindIII/BamHI fragment with HindIII/BamHI digested pTRP3. pTRP3 is a pBR322 based vector containing the trp promoter with a downstream HindIII site; pTRP3 was deposited with ATCC 18 December 1984, and has accession no. 39946.

pRAP229 was constructed using coding sequences 20 derived entirely from pRATI. It was obtained by a three-way ligation of the large NarI/BamHI repliconcontaining fragment of pSYC1089 which provides, in order. B. thurinqiensis-positive retroregulator sequences, the chloramphenicol resistance marker, a compatible replicon, and the phoA promoter and leader sequences; ClaI/BamHI-digested pRATI which provides a 500 bp fragment encoding the C-terminal portion of ricin A properly terminated: and the N-terminal sequence as provided by an approximately 350 bp Clal/ClaI frag- 30 ment from pRAT1. It is clear that the ricin A sequences could also have been. and might preferably be, prepared as a ClaI(partial)/BamHI-excised fragment from pRATI.

The resulting fusion retains the start codon of the ricin A chain preceding the isoleucine residue; is separated by 7 bp and thus out of reading frame relative to the leader sequence: extends the phoA leader by the tripeptide Ile-Ser-Leu; and (4) allows for termination of the leader sequence at a TGA codon out of frame with, but proximal to, the start codon of ricin A. pRAP229 was deposited at ATCC on 8 March 1985 and has accession no. 53408.

D.7. Production and Processing of Ricin A in E. coli E. coli MM294 was transformed either with pRAP229 alone or cotransformed with pRAP229 and pSYC1174. The transformed cultures were grown under conditions similar to those described by Michaelis, et al, J Bact (1983) 154:356-365. The cells were induced by lowering the exogenous phosphate concentration and maintaining the cultures for 16-17 hr.

The cells were harvested, and whole cell extracts prepared by sonication in the absence of detergent were assayed for expression using Western blot a 20 employing rabbit antisera to native ricin A. To assess the N-terminal methylation, the ricin A was purified and subjected to Edman degradation for quantitative analysis. When the cells were transformed with pRAP229 alone, 40% of the ricin A contained an N-terminal methionine; the cotransformed cells produced ricin A 0 having only 9% of the chains methylated.

D.8. In Vitro Processing of Met-Ricin A o Purified ricin A (600 jig) from the pRAP229 o 30 transformed cell lysates was mixed with 24 jig of Metaminopeptidase purified from E. coli pSYC1174 in 0.2 mM cobalt chloride and 0.1 mM potassium phosphate buffer.

pH 7.5, having 0.3 ml total volume. The reaction mixtures were incubated overnight at 30 0 C and stopped by -36heating in a boiling water bath. The N-terminal sequence was determined by Edman degradation after desalting the reaction mixture. Control mixtures containing no Met-aminopeptidase showed 40% of the ricin A with N-terminal methionine. the same fraction normally found in the lysate, as described above. Reaction mixtures containing the Met-aminopeptidase enzyme contained ricin A wherein only 8% of the protein contained N-terminal methionine, substantially the same fraction as obtained in pRAP229/pSYC1174 transformed cells.

On 27 August 1985, E. coli strain pSYC1174 was deposited with the American Type Culture Collection (ATCC 53245) under the terms of the Budapest Treaty on the International Recognition of the Deposit of Microorganisms for the Purposes of Patent Procedure and the 0 Regulations thereunder (Budapest Treaty). This assures maintenance of a viable culture for 30 years from date of deposit. The organisms will be made available by o 1 20 ATCC under the terms of the Budapest Treaty, and subject to an agreement between Applicants and ATCC which assures unrestricted availability upon issuance of the pertinent U.S. patent. Availability of the deposited o strains is not to be construed as a license to practice the invention in contravention of the rights granted 4o o under the authority of any government in accordance with its patent laws.

Claims (19)

1. A method to obtain a DNA sequence encoding a bacterial Met- aminopeptidase, wherein said Met-aminopeptidase has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues, and does not cleave at other N-terminal residues, and wherein said Met-aminopeptidase releases methionine from a peptide selected from the group consisting of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; Met-Ala-Ser; Met-Gly-Gly; Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gln-Leu; and Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys; and releases no amino acids from a peptide selected from the group consisting of: Met-Phe-Gly; Met-Phe-Ala-Gly; Met-Leu-Phe; SMet-Met-Met; Leu-Leu-Leu; Leu-Gly-Gly; Met-Ala; .0t' S. Leu-Gly; .O Leu-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gln-Leu; N-formyl-Met-Met-Met; 0 Met-Phe; Met-Ser; Val-Gly-Gly; o 0° .Thr-Gly-Gly; o"o o Trp-Gly-Gly; Phe-Gly-Gly; Met-Glu-His-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 -Gly; TMR/947u 38 Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Gln-Leu-Cys; Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu; Thr-.Val-Leu; Arg-Gly-Gly; Ala-(Ala) -Ala; 2 Ala-Ala-Ala; Glu-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and Met-Arg-Phe acetate; which method comprises: preparing a plasmid-borne gene/library from a first bacterial strain; l transforming said gene library into a second bacterial strain that is deficient in general peptidase activity; screening transformants DNA from transformants having said activity.

2. The method of claim 1 wherein the first bacterial strain is deficient in peptidase activity.

3. The method of claim 2 wherein the first bacterial strain and second bacterial strain are the same.

4. A method to obtain a DNA sequence encoding a bacterial Met- aminopeptidase, wherein said Met-aminopeptidase has a specificity whereby S it effects cleavage of the N-terminal methionine residue from Met-preceded S peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues and wherein said Met- aminopeptidase releases methionine from a peptide selected from the group S consisting of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; Met-Ala-Ser; Met-Gly-Gly; Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Thr-Gln-Leu; and TMR/947u 0 *0 0* Lt4, o 0 00 39 Met-Pro-Thr-Ser-Ser-Ser-Th--Lys-Lys-Gl n-Leu-Cys; and rel eases no ami no acids from a peptide selected from the group consisting of: Met-Phe-Gly; Met-Phe-Al a-Gly; Met-Leu-Phe; Met-Met-Met; Leu-Leu-Leu; Leu-Gly-Gly; Met-Ala; Leu-Gly; Leu-Al a-Pro-Thr-Ser--Ser-Ser-Tlr-Lys-Lys-Thr-Gl n-Leu; N-formyl -Met-Met-Met; Met-Phe; Met-Ser; Val-Gly-Gly; Thr-Gly-Gly; Trp-Gly-Gly; Met-Gl u-Hi s-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Prc/-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 Gly; Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gl n-Leu-Cys; Al a-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gl n-Leu; Thr-Val -Leu; Arg-Gly-Gly; Al a-(Al a) 2 Ala; Ala-Ala-Ala; Gl u-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and Met-Arg-Phe acetate; which method comprises: screening bacterial transformants for Met-aminopeptide activity, and recovering plasmid DMA from transformants having such activity; wherein the transformants were prepared by 0 .0 6 TMR/947u 40 preparing a plasmid-borne gene library from a first bacterial strain; and transforming said gene library into a second bacterial strain that is deficient in general peptidase activity. The method of claim 4 wherein the first bacterial strain is deficient in peptidase activity.

6. The method of claim 5 wherein the first bacterial strain and the second bacterial strain are the same.

7. The method of claim 6 wherein the bacterial strain is E. coli CM89 as hereinbefore defined.

8. A recombinant bacterium which contains an expression system functional in expressing DNA encoding Met-aminopeptidase, wherein said Met- aminopeptidase has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, wherein the Met-aminopeptidase releases methionine from a peptide selected from the group consisting of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; Met-Ala-Ser; Met-Gly-Gly; Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gln-Leu; and Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys; and releases no amino acids from a peptide selected from the group consisting of: Met-Phe-Gly; S0| Met-Phe-Ala-Gly; Met-Leu-Phe; Met-Met-Met; 9oo Leu-Leu-Leu; o"'o Leu-Gly-Gly; Met-Ala; Leu-Gly; Leu-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-G1n-Leu; N-formyl-Met-Met-Met; TMR/9471 41 Met-Phe; Met-Ser; Val-Gly-Gly; Thr-Gly-Gly; Trp-Gly-Gly; Phe-Gly-Gly; Met-Glu-His-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 -Gly; Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Gln-Leu-Cys; Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu; Thr-Val-Leu; Arg-Gly-Gly; Ala-(Ala) 2 -Ala; Ala-Ala-Ala; Glu-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and Met-Arg-Phe acetate; and an expression system functional in expressing the DNA encoding a Met-preceded desired recomblnant foreign protein.

9. A method for producing an N-terminal Met-less recombinant S protein in a bacterial host which method comprises: o, culturing a recombinant bacterium which contains an expression system functional in expressing DNA encoding Met-aminopeptidase which effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, wherein the Met-aminopeptidase methionine releases methionine from a peptide selected from the group *o o consisting of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; TMR/947u -42- Met-Al a-Ser; Met-Gly-Gly; Met-Al a-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gl n-Leu; and Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys; and releases no amino acids from a peptide selected from the group consisting of: Met-Phe-Gly; Met-Phe-Al a-Gly; Met-Leu-Phe; Met-Met-Met; Leu-Leu-Leu; Leu-Gly-Gly; Met-Ala; Leu-Gly; Leu-Al a-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gl n-Leu; N-formyl -Met-Met-Met; Met-Phe; Met-Ser; Val-Gly-Gly; Thr-Gly-Gly; Trp-Gly-Gly; Phe-Gly-Gly; Met-Gl u-Hi s-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 -Gly; Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Trhr-Lys-Lys-Gl n-Leu-Cys; Al a-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gl n-Leu; Thr-Val-Leu; Arg-Gly-Gly; Ala-(Ala) 2 -Ala; a Ala-Ala-Ala; Gi u-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and TMR/947u 43 Met-Arg-Phe acetate; and an expression system functional in expressing the DNA encoding a Met-preceded desired recombinant foreign protein, under conditions appropriate for the expression of said DNAs encoding said Met-amino- peptidase and said desired recombinant foreign protein. A method to prepare N-terminal methionine-free protein which comprises treating a Met-preceded protein with an effective amount of Met- aminopeptidase, wherein said Met-aminopeptidase is prepared by culturing transformant cells; which cells have been transformed with a recombinant DNA expression system comprising control sequences operably linked to DNA encoding Met- aminopeptidase, wherein said Met-aminopeptidase has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the group consisting of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; Met-Ala-Ser; Met-Gly-Gly; Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Thr-Gln-Leu; and Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys; and releases no amino acids from a peptide selected from the group consisting of: Met-Phe-Gly; o Met-Phe-Ala-Gly; Met-Leu-Phe; Met-Met-Met; Leu-Leu-Leu; Leu-Gly-Gly; Met-Ala; Leu-Gly; Leu-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gln-Leu; N-formyl-Met-Met-Met; Met-Phe; TMR/947u II.I--I -i 44 Met-Ser; Val-Gly-Gly; Thr-Gly-Gly; Trp-Gly-Gly; Phe-Gly-Gly; Met-Glu-His-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 -Gly; Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Gln-Leu-Cys; Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu; Thr-Val-Leu; Arg-Gly-Gly; Ala-(Ala) 2 -Ala; Ala-Ala-Ala; Glu-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and Met-Arg-Phe acetate; said culturing under conditions which favor expression of said DNA encoding Met-aminopeptidase; and recovering Met-aminopeptidase from the transformants.

11. The method of claim 10 wherein the Met-aminopeptidase is derived from E. coll, and the Met-preceded protein Is IL-2. pl? 12. The method of claim 11 wherein the E. coli is strain pSYC1174 (as hereinbefore described). "13. The method of claim 10 wherein the Met-aminopeptidase is derived from E. coli, and the Met-preceded protein is ricin A.

14. The method of claim 10 wherein the DNA encoding Met-amino- o peptidase is obtainable by a process comprising: a preparing a plasmid borne gene library from a first bacterial strain; transforming said gene library into a second bacterial strain that is deficient in peptidase activity; screening transformants for Met-aminopeptidase activity; and recovering plasmid DNA from transformants having said activity. TMR/947u i 45 The method of claim 10 wherein the DNA encoding Met-amino- peptidase is obtainable by a process comprising: screening bacterial transformants for Met-aminopeptidase activity and recovering plasmid DNA from transformants having such activity; wherein the transformants were prepared by preparing a plasmid borne gene library from a first bacterial strain; and transforming said gene library into a second bacterial strain that is deficient in peptidase activity.

16. The method of claim 10 wherein the DNA encoding Met-amino- peptidase is obtainable by a process comprising screening a microbial genomic library with a labeled DNA probe comprising the DNA of Figure 2 encoding amino acids 1-264 of that figure or its complement, and recovering the DNA which hybridizes to said probe.

17. A Met-aminopeptidase in purified and isolated form characterized in that it has a specificity whereby it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the group consisting of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; Met-Ala-Ser; o Met-Gly-Gly; Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Thr-Gln-Leu; S and Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys; and releases no amino acids from a peptide selected from the group consisting of: Met-Phe-Gly; Met-Phe-Ala-Gly; Met-Leu-Phe; Met-Met-Met; Leu-Leu-Leu; Leu-Gly-Gly; Met-Ala; Leu-Gly; TMR/47AN TMR/947u 4. 0 46 Leu-Al a-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-G n-Leu; N-formyl-Met-Met-Met; Met-Phe; Met-Ser; Val-Gly-Gly; Thr-Gly-Gly; Trp-Gly-Gly; Phe-Gly-Gly; Met-Glu-His-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 -Gly; Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Gln-Leu-Cys; Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu; Thr-Val-Leu; Arg-Gly-Gly; Ala-(Ala) 2 -Ala; Ala-Ala-Ala; Glu-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; ,oe Ile-Gly-Gly; and S Met-Arg-Phe acetate.

18. The Met-aminopeptidase of claim 17 which is encoded by a DNA S which hybridizes to a labeled DNA comprising the DNA of Figure 2 encoding amino acids 1-264 of that figure or its complement, under hybridization conditions that are equivalent in stringency to hybridization in a buffer containing 6 x SSC, 0.01 M EDTA, 5 x Denhardt's, 0,5% SDS at 65 0 C for sufficient time to complete reaction, followed by washing with 3 x SSC at o o

19. The Met-aminopeptidase of claim 18 which has the amino acid sequence shown in Figure 2. An antibody composition immunoreactive with the Met-amino- peptidase of claims 17-19.

21. An isolated DNA encoding an aininopeptidase wherein said Met-aminopeptidase has a specificity wherein it effects cleavage of the TMR/947u 47 N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the group consisting of: Met-Ala-Met; Met-Gly-Met-Met; Met-Gly-Met; Met-Al a-Ser; Met-Gly-Gly; Met-Al a-Pro-Thr-Ser--Ser-Ser-Thr-Lyr-Lys-Thr-G1 n-Leu; and Met-Pr-o-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys; and releases no amino acids from a peptide selected from the group consisting of: 0400e- ly Met-Phe-AGly; Met-Leu-Phe; Met-Met-Met; I. Leu-Leu-Leu; Leu-Gly-Gly; Met-Ala; Leu-Gly; 0 0 aLeu-Al a-Pro-Thr-Ser-Ser--Ser-Thr-Lys-Lys-Thr-Gl ri-Leu; N-formyl -Met-Met-Met; o Met-Phe; Met-Ser; Val-Gly-Gly; o Thr-Gly-Gly; 0 Trp-Gly-Gly; vo o Phe-Gly-Gly; Met-Gl u-Hi s-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 Gly; Ser-Ser-Ser; Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Gl n-Leu-Cys; Al a-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gl n-Leu; Thr-Val -Leu; TMR/947u ,d ru i 48 Arg-Gly-Gly; Ala-(Ala) 2 -Ala; Ala-Ala-Ala; Glu--Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and Met-Arg-Phe acetate.

22. The DNA of claim 21 which hybridizes to a labeled DNA comprising the DNA of Figure 2 encoding amino acids 1-264 of that figure or its complement, under hybridization conditions that are equivalent in stringency to hybridization in a buffer containing 6 x SSC, 0.01 M EDTA, x Denhardt's, 0.5% SDS at 65 0 C for sufficient time to complete reaction, followed by washing with 3 x SSC at

23. An expression system capable, when contained in a recombinant host, of expression a DNA encoding a Met-aminopeptidase which has a specificity wherein it effects cleavage of the N-terminal methionine residue from Met-preceded peptides or proteins without cleavage of internal methionine residues and does not cleave at other N-terminal residues, and wherein methionine is released from a peptide selected from the group consisting of: Met-Ala-Met; S. Met-Gly-Met-Met; Son Met-Gly-Met; o Met-Ala-Ser; 0 Met-Gly-Gly; o o Met-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Thr-Gln-Leu; and Met-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu-Cys; and releases no 0 amino acids from a peptide selected from the group consisting of: Met-Phe-Gly; Met-Phe-Ala-Gly; Met-Leu-Phe; Met-Met-Met; Leu-Leu-Leu; Leu-Gly-Gly; TMR/947u 49 Met-Ala; Leu-Gly; Leu-Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Thr-Gln-Leu; N-formyl-Met-Met-Met; Met-Phe; Met-Ser; Val-Gly-Gly; Thr-Gly-Gly; Trp-Gly-Gly; Phe-Gly-Gly; Met-Glu-His-Phe-Arg-Tyr-Gly; Met-Lys-Arg-Pro-Pro-Gly-Phe-Ser-Pro-Phe-Arg; Gly-(Gly) 3 -Gly; Ser-Ser-Ser; 'Pro-Thr-Ser-Ser-Ser-Thr-Lyr-Lys-Gln-Leu-Cys; Ala-Pro-Thr-Ser-Ser-Ser-Thr-Lys-Lys-Gln-Leu; Thr-Val-Leu; Arg-Gly-Gly; Ala-(Ala) 2 -Ala; Ala-Ala-Ala; Glu-Gly-Phe; Leu-Leu-Leu; Tyr-Gly-Gly; Ile-Gly-Gly; and Met-Arg-Phe acetate.

24. The expression system of claim 23 wherein said encoding DNA hybridizes to a labeled DNA comprising the DNA of Figure 2 encoding amino acids 1-264 of that figure or its complement, under hybridization in a buffer containing 6 x SSC, 0.01 M EDTA, 5 x Denhardt's, 0.5% SDS at S for sufficient time to complete reaction, followed by washing with 3 x SSC at 65 0 C. A recombinant host which has been modified to contain the expression system of claim 23 or 24.

26. A method to prepare a recombinant Met-aminopeptidase which comprises: TMR/947u ~I 50 culturing a recombinant host containing the expression system of claim 23 or 24 under condition for expression of the DNA encoding the Met-aminopeptidase, and recovering the Met-aminopeptidase from the culture. DATED this SEVENTEENTH day of OCTOBER 1989 Cetus Corporation Patent Attorneys for the Applicant SPRUSON FERGUSON 4OU 0 4 4 4; o I '4 001 004 4 0 4 0 9) A. u TMR/947u